Immunolocalization and in vivo Functional Analysis by RNAi of the Aedes Kinin Receptor in Female Mosquitoes of Aedes aegypti (L.) (Diptera, Culicidae)

Kersch, Cymon

2011 December 1900

The evolution of the blood feeding adaptation has required precise coordination of multiple physiological processes in the insect, such as reproduction, behavior, digestion and diuresis. These processes are under careful synchronous hormonal control. For rapid excretion, multiple diuretic hormones are known. Although originally described based on their ability to stimulate hindgut contractions, the Aedes kinins have been shown to stimulate fluid secretion in female mosquitoes of Aedes aegypti. Aedes kinins are leucokinin-like neuropeptides released from neurosecretory cells in the brain and abdominal ganglia. They act by binding to the Aedes kinin receptor, a G proteincoupled receptor (GPCR). The Aedes kinin receptor has been cloned, sequenced, functionally characterized, and immunolocalized to stellate cells in the Malpighian tubules of Ae. aegypti. In addition to their myotropic and diuretic roles, leucokinin-like peptides and/or their receptors have been also been discovered in the nervous, digestive, and reproductive systems of other arthropod species. Therefore, the Aedes kinins have the potential to function in several simultaneous physiological processes that are stimulated by blood feeding. This thesis aims to understand better their role in the whole mosquito by investigating the Aedes kinin receptor's global expression as well as its in vivo contribution to post-prandial diuresis. Presence of the Aedes kinin receptor was investigated in the head, posterior midgut (stomach), hindgut, ovaries, and Malpighian tubules of both non blood-fed and blood-fed females by western blot using anti-receptor antibodies. The receptor was then immunolocalized in the posterior midgut and rectum. Finally, RNAi was employed to knock down kinin receptor expression, followed by measurement of in vivo urine excretion post blood feeding in a precision humidity chamber. Transcript and protein knockdown were confirmed by qPCR and immunohistochemistry, respectively. Results indicate widespread expression of the Aedes kinin receptor protein in organs novel for hematophagous insects and demonstrate the receptor's fundamental role in rapid diuresis. These findings strongly point to the Aedes kinins as integrative signaling molecules that could coordinate multiple physiological systems. The Aedes kinins could therefore have contributed to the success of the blood feeding adapation in mosquitoes.

leucokinin

insect GPCR (G protein-coupled receptor)

diuresis

Malpighian tubules

RNAi

rectum

midgut

mosquito blood feeding.

The Evolutionary History of Vertebrate Adhesion GPCRs and Its Implication on Their Classification

Wittlake, Aline, Prömel, Simone, Schöneberg, Torsten

23 January 2024

Adhesion G protein-coupled receptors (aGPCRs) form a structurally separate class of GPCRs with an unresolved evolutionary history and classification. Based on phylogenetic relations of human aGPCRs, nine families (A–G, L, V) were distinguished. Taking advantage of available genome data, we determined the aGPCR repertoires in all vertebrate classes. Although most aGPCR families show a high numerical stability in vertebrate genomes, the full repertoire of family E, F, and G members appeared only after the fish–tetrapod split. We did not find any evidence for new aGPCR families in vertebrates which are not present in the human genome. Based on ortholog sequence alignments, selection analysis clearly indicated two types of tetrapod aGPCRs: (i) aGPCR under strong purifying selection in tetrapod evolution (families A, B, D, L, V); and (ii) aGPCR with signatures of positive selection in some tetrapod linages (families C, E, G, F). The alignments of aGPCRs also allowed for a revised definition of reference positions within the seven-transmembranehelix domain (relative position numbering scheme). Based on our phylogenetic cluster analysis, we suggest a revised nomenclature of aGPCRs including their transcript variants. Herein, the former families E and L are combined to one family (L) and GPR128/ADGRG7 forms a separate family (E). Furthermore, our analyses provide valuable information about the (patho)physiological relevance of individual aGPCR members.

info:eu-repo/classification/ddc/610

ddc:610

Modulation orthostérique et allostérique du PAFR par des molécules synthétiques

Noël, Cynthia Jenny

January 2008

Le PAF (facteur d'activation des plaquettes) est un médiateur lipidique de l'inflammation très puissant impliqué dans plusieurs conditions pathophysiologiques.Le PAF agit principalement via un seul récepteur, le PAFR qui appartient à la famille des récepteurs couplés aux protéines G, les GPCRs. Le"two state model" assume que les GPCRs existent dans un état d'équilibre entre un état inactif (R) et un état actif (R*). L'isomérisation de R vers R* peut arriver de façon spontanée, c'est à dire indépendamment de la liaison d'un agoniste. Dans ces travaux de recherche, nous avons tenté de déterminer la propriété antagoniste et agoniste inverse des molécules orthostériques (WEB2086, PCA4248, FR49175, bromure d'octylonium, CV3988 et le Trans BTP dioxolane) à activer la voie des MAPK ainsi que le cycle biochimique des inositols phosphates dans la lignée cellulaire HEK 293 transfectée de façon stable avec le récepteur du PAF. De plus, l'activité potentiellement allostérique sur le PAFR de modulateurs synthétiques tels le THG-315, le THG-316 et MAREK a également été investiguée dans la même lignée cellulaire. Finalement, des surnageants d'hybridome 9H1/1C1, 9F5/1H4, 9F5/1H4, 9F5/1F8, 9F5/2B3 et 9F5/2E4 contenant des anticorps monoclonaux, dirigés tous contre un peptide qui équivaut à la région C-terminale de la troisième boucle extracellulaire du PAFR: GFQDSKfHQA ont également été utilisés, afin : (1) de déterminer le meilleur clone en terme d'affinité et de spécificité et (2) effectuer des tests pour savoir s'ils possèdent des propriétés agonistes ou antagonistes sur le PAFR. En conclusion, les résultats obtenus nous indiquent que : (1) l'efficacité des molécules orthostériques à antagoniser les réponses induites par le PAF dépend de leur nature et de leur concentration, (2) les modulateurs potentiellement allostériques utilisés ne modulent aucune des voies majoritairement connues pour être activées par le PAFR, et (3) qu'il n'y a aucun marquage spécifique du PAFR avec les surnageants d'hybridomes utilisés.

Activation orthostérique

GPCR (G protein coupled receptor)

PAF (platelet activating factor)